Abstract
Cortical columns are the functional units of the neocortex that are particularly prominent in the “barrel” field of the somatosensory cortex. Here we describe the morphology of two classes of synaptically coupled excitatory neurons in layer 4 of the barrel cortex, spiny stellate, and star pyramidal cells, respectively. Within a single barrel, their somata tend to be organized in clusters. The dendritic arbors are largely confined to layer 4, except for the distal part of the apical dendrite of star pyramidal neurons that extends into layer 2/3. In contrast, the axon of both types of neurons spans the cortex from layer 1 to layer 6. The most prominent axonal projections are those to layers 4 and 2/3 where they are largely restricted to a single cortical column. In layers 5 and 6, a small fraction of axon collaterals projects also across cortical columns. Consistent with the dense axonal projection to layers 4 and 2/3, the total number and density of boutons per unit axonal length was also highest there. Electron microscopy combined with GABA postimmunogold labeling revealed that most (>90%) of the synaptic contacts were established on dendritic spines and shafts of excitatory neurons in layers 4 and 2/3.
The largely columnar organization of dendrites and axons of both cell types, combined with the preferential and dense projections within cortical layers 4 and 2/3, suggests that spiny stellate and star pyramidal neurons of layer 4 serve to amplify thalamic input and relay excitation vertically within a single cortical column.
- barrel cortex
- layer 4
- spiny stellate cell
- star pyramidal neuron
- cortical column
- axonal projection
- paired recordings
- intracellular labeling
Sensory cortices display a distinctive organization into functional modules of neuronal ensembles, the so-called cortical columns that process signals from the periphery (Mountcastle, 1957; Mountcastle and Powell, 1959; Hubel and Wiesel, 1962; for review, see Mountcastle, 1997; Rockland, 1998). One striking example of such a modular organization is the “barrel” field in the somatosensory cortex of rodents. In layer 4 of the barrel cortex, each whisker hair on the animal's muzzle is topographically represented in a one-to-one relationship (Woolsey and van der Loos, 1970; Welker, 1976; for review, see Juliano and Jacobs, 1995).
In sensory cortices, layer 4 is the main input region for afferent fibers originating in the respective thalamic relay nuclei (Hubel and Wiesel, 1962; McGuire et al., 1984; Chiaia et al., 1991a,b; for review, see Sherman and Guillery, 1996). Although a small fraction (∼20%) of these thalamic afferents terminate on aspinous, presumably GABAergic interneurons (White and Rock, 1981; White et al., 1984; Benshalom and White, 1986), their main target cells are excitatory spiny neurons in layer 4. Most of these neurons resemble spiny stellate cells, whereas a smaller fraction has been described as star pyramidal cells (Lund, 1984; Ahmed et al., 1994; Hirsch, 1995). Thus, these neurons are the first elements involved in intracortical signal processing (Mountcastle and Powell, 1959; Hubel and Wiesel, 1962; LeVay, 1973; Martin and Whitteridge, 1984; McGuire et al., 1984; Douglas and Martin, 1991;Armstrong-James et al., 1992; for review, see McCormick, 1992).
An understanding of the function of spiny neurons in layer 4 in the microcircuitry of a cortical column requires detailed knowledge about their anatomical organization, in particular their axonal projections and their postsynaptic target cells. Earlier Golgi studies described the dendritic morphology of spiny neurons in rodent barrel cortex (Pasternak and Woolsey, 1975; Woolsey et al., 1975; Steffen, 1976;Steffen and van der Loos, 1980; Harris and Woolsey, 1981; Simons and Woolsey, 1984; for review, see Juliano and Jacobs, 1995) but lacked information about the axonal projections at the single-cell level and the target cells of these neurons. However, small extracellular biocytin deposits revealed that most of the projections are to supragranular layers, and relatively few direct connections exist between hollows of neighboring barrels (Kim and Ebner, 1999).
Here we have used dual whole-cell recordings from pairs of neurons combined with reconstruction of the biocytin-filled neurons to quantitatively describe the dendritic arborization and in particular the axonal projections and the postsynaptic target structures of synaptically coupled spiny neurons in layer 4 of rat barrel cortex. We show that the dendritic arbor is largely confined to a single barrel in layer 4 and that the axon projects vertically throughout all cortical layers but remains predominantly within the same cortical column. In conjunction with the functional properties of these connections (Feldmeyer et al., 1999b), the largely columnar organization of the axons suggests that as an ensemble, excitatory spiny neurons in layer 4 serve to amplify thalamic inputs and relay excitation to superficial laminae within a cortical column. Therefore, spiny layer 4 neurons act as the principal gate for the signal flow within a cortical column.
MATERIALS AND METHODS
Preparation of acute brain slices. All experiments were performed in accordance with the animal welfare guidelines of the Max-Planck Society and the University of Freiburg. Wistar rats (12–22 d old) were anesthetized with halothane and decapitated, and slices through the somatosensory cortex were cut in cold extracellular solution using a vibrating microslicer (DTK-1000, Dosaka Co. Ltd., Kyoto, Japan) and prepared according to methods described elsewhere (Agmon and Connors, 1991; Feldmeyer et al., 1999b). Slices (350–400 μm thick) were collected, incubated at 35°C in extracellular solution for 30–60 min, and subsequently maintained at room temperature (20–23°C) before electrical recordings were made.
Solutions. Slices were continuously superfused with extracellular solution containing (in mm): 125 NaCl, 2.5 KCl, 25 glucose, 25 NaHCO3, 1.25 NaH2PO4, 2 CaCl2 and 1 MgCl2 bubbled with 95% O2 and 5% CO2. The intracellular pipette solution contained (in mm): 105 K-gluconate, 30 KCl, 10 HEPES, 10 phosphocreatine, 4 ATP-Mg, 0.3 GTP (adjusted to pH 7.3 with KOH). The osmolarity of this solution was 300 mOsm. For subsequent morphological analysis, 2–5 mg/ml biocytin (Sigma, München, Germany) was routinely added to the internal solution, and neurons were filled during 1–3 hr of recording.
Identification of synaptically connected neurons in layer 4 of the barrel cortex. Slices of rat somatosensory cortex were placed in the recording chamber under an upright microscope (Axioskop Carl Zeiss Göttingen, Germany) fitted with 2.5× plan/0.075 NA and 40×-W/0.80 objectives) with the pial surface pointing to the front and the hippocampus to the right. The barrel field was visualized at low magnification under bright-field illumination and can be identified in layer 4 as evenly spaced dark structures. Barrel structures are present in five to six slices but a continuous band of barrels is visible only in two to three slices just above the hippocampus, fimbria-fornix, and lateral ventricle. Individual layer 4 neurons were identified at 40× magnification using infrared-differential interference contrast (IR-DIC) microscopy as previously described. The somata of layer 4 neurons in the barrel field tended to be organized in clusters in the dark edges of a barrel (see Fig. 1B,C) when compared with the light centers.
Electrophysiological recordings. Whole-cell voltage recordings from presynaptic and postsynaptic spiny layer 4 neurons were made as described elsewhere (Feldmeyer et al., 1999b). In brief, a postsynaptic cell was recorded from with one pipette, and subsequently synaptic connections to this cell were searched with a second pipette in the loose-patch configuration. When EPSPs in response to the loose-patch stimulation were detected in the postsynaptic neuron, the presynaptic cell was repatched with a new pipette filled with biocytin-containing intracellular solution using the whole-cell (voltage recording) mode. Potentials were amplified using an EPC9–2 (for dual whole-cell recording; HEKA Elektronik Lambrecht). Recordings were filtered at 2–5 kHz, digitized at 5–10 kHz using an ITC-16 interface (Instrutech, Great Neck, NY), and stored on the hard disk of a Macintosh or a PC.
Histological procedures. After recording and loading with biocytin, brain slices were fixed in 100 mmphosphate-buffered (PB) solution, pH 7.4, containing 1% paraformaldehyde and 2.5% glutaraldehyde at 4°C for at least 24 hr. Endogenous peroxidase was blocked by incubation of the slices in 1% H2O2 for 15–20 min. After several rinses in PB solution they were then transferred to a 1% avidin–biotinylated horseradish peroxidase complex containing 0.1% Triton X-100 (ABC-Elite Camon, Wiesbaden, Germany) and left overnight at 4°C while shaking slightly. The next day, slices were reacted using 3,3-diaminobenzidine (DAB; Sigma) and 0.01% H2O2 until dendrites and axonal arbors were clearly visible (after approximately 2–5 min). Slices were mounted on glass slides, embedded in Moviol (Hoechst AG, Frankfurt AM, Germany), and coverslipped.
Individual selected spiny stellate (n = 2) and star pyramidal neurons (n = 1) were processed for electron microscopic analysis to identify the postsynaptic target structures of these neurons. After cryoprotection in 10% (20 min) and 20% (30 min) sucrose, sections were freeze-thawed in liquid nitrogen. After several rinses in PB solution, sections were incubated overnight in ABC solution and reacted as described above. To enhance staining contrast, slices were post-fixed in 0.5% OsO4 (30–45 min), then dehydrated and embedded in Durcupan (Fluka, Deisenhofen, Germany). Serial ultrathin sections through the entire axonal domain were cut with an ultramicrotome (Leitz-Ultracut, Hamburg, Germany), counterstained, and examined with a Philips CM 100 electron microscope (Philips, Eindhoven, The Netherlands).
GABA postembedding immunogold labeling. The immunogold staining procedure was performed as described by Somogyi and Hodgson (1985), using a commercially available antiserum against GABA (Sigma). The immunostaining was performed on droplets of Millipore-filtered solutions in humid Petri dishes. Immersion in 1% periodate (10 min) was followed by several washes in double-distilled water. Thereafter, the grids were transferred through 2 or 5% sodium metaperiodate (10–30 min) and rinsed several times in double-distilled water and three times in Tris-buffered saline (TBS), pH 7.4. After preincubation in 1% ovalbumin dissolved in TBS (30 min), the grids were incubated in rabbit anti-GABA antiserum (1:5000, in 1% normal goat serum in TBS). After rinsing in TBS and 50 mm Tris buffer, pH 7.4, containing 1% bovine serum and 0.5% Tween 20 (10 min), the grids were incubated in the secondary antibody (goat anti-rabbit IgG-coated colloidal gold, 10 nm) for 2 hr (diluted 1:10, in darkness). After rinsing in 2% glutaraldehyde (10 min), the grids were washed again in double-distilled water and stained with uranyl acetate and lead citrate. In control experiments without the primary antibody and sections processed for GABA postimmunogold labeling, almost no or only low background labeling was detected, whereas labeling of structures presumed to be GABAergic exceeded the mean gold particle density of the maximal background staining by at least four SDs.
Morphological reconstructions of biocytin-filled synaptically coupled neurons. Biocytin-labeled pairs of synaptically coupled neurons were examined under the light microscope at high magnification. Only pairs for which a complete physiological analysis was made and that had no obvious truncation of their dendritic and axonal profiles were used for qualitative and quantitative morphology. Measurements were not corrected for shrinkage. Representative neuron pairs were photographed at various magnifications to document dendritic morphology, axonal projection, and location of synaptic contacts. The outline of neurons was then drawn with the aid of a camera lucida attached to an Olympus BX50 microscope (Olympus, Hamburg, Germany) at a final magnification of 720×. For some pairs of neurons, three-dimensional reconstructions were also made at 400× magnification using the Neurolucida (Microbrightfield, Colchester, UK) software. The reconstructions provided the basis for further quantitative morphological analysis of the following parameters: (1) maximal horizontal field span of the dendrites and axons, (2) total number and distribution of putative synaptic contacts per neuron, (3) total number of boutons in cortical layers 1 to 6, and (4) number of boutons per 100 μm of axonal segment counted separately for each cortical layer. For all data, means ± SD were calculated. Significance was tested using a two-tailed Student's ttest.
Cytochrome oxidase histochemistry. To identify the barrel structure in layer 4 of the somatosensory cortex, the cytochrome oxidase staining according to Wong-Riley (1979) was used on perfusion-fixed rat brains of the same age (postnatal day 12–15) as used for the acute slice preparations. In brief, animals were perfused transcardially with a PB solution containing 4% paraformaldehyde. Brains were stored overnight in the same fixative at 4°C and then prepared as described above. After several rinses in PB solution, free-floating 100-μm-thick vibratome sections through the barrel field were incubated in a PB solution containing 50 mg DAB, 15–30 mg cytochrome c, and 20 mg catalase/100 ml at 37°C for 2 hr in the dark. The reaction was stopped when individual barrels were clearly distinguishable from the background (see Fig.1A). After several rinses in PB solution, sections were mounted on glass slides, air-dried, defatted in absolute alcohol and xylene, finally embedded in Hyper-Mount (Life Science, Frankfurt, Germany), and coverslipped. In some experiments, cytochrome oxidase histochemistry and labeling of single biocytin-filled neurons (n = 15 neurons) were combined to reveal the dendritic and axonal organization with respect to the barrel structure (see Fig.2B, inset, D).
RESULTS
Cytochrome oxidase stain of the barrel cortex slices
All experiments were performed on thalamocortical slices in which the barrel structure in layer 4 is easily recognizable. Figure1A illustrates the barrel structure in somatosensory cortex as revealed by cytochrome oxidase staining that mirrors the bright-field images taken from acute slice preparations of the barrel cortex. Combined bright-field and IR-DIC videomicroscopy at low and high magnification, respectively, showed that the somata of neurons appeared to be organized in clusters of 5–15 neurons (Fig.1B,C), with a predominant location at the edges of individual barrels. In contrast, spiny stellate neurons in the visual cortex display a more homogeneous distribution throughout layer 4 (LeVay, 1973; Lund, 1984; Martin and Whitteridge, 1984, 1988).
Multiple biocytin labeling of individual neurons in combination with cytochrome oxidase staining (n = 15 neurons) revealed that almost the entire dendritic and axonal domain of excitatory spiny neurons in layer 4 was confined to a single cortical column. This was found for all spiny layer 4 neurons in the barrel field (Fig.2A,B). In contrast, layer 5 pyramidal neurons (n = 5) injected right below the barrels showed a completely different morphology, and their apical dendrites showed no obvious relationship to the barrels as defined with cytochrome oxidase staining (Fig.2C,D).
Morphology of synaptically coupled spiny layer 4 neurons
Excitatory layer 4 neurons were identified by their shape in IR-DIC and their “regular” pattern of action potentials after current injection (Connors and Gutnick, 1990; Feldmeyer et al., 1999b). Spiny layer 4 neurons, i.e., spiny stellate and star pyramidal cells, were easily distinguished by their spherical to ovoid somata and the absence of a prominent apical dendrite (Fig. 1C). In addition, their somata appeared to be larger than those of GABAergic aspiny stellate layer 4 interneurons (≥10 vs ≤10 μm) but smaller than that of GABAergic interneurons with fusiform somata (>20 μm). Monosynaptic connections between spiny layer 4 neurons were reliable and characterized by a low coefficient of variation and a low failure rate of unitary EPSPs (Feldmeyer et al., 1999b).
From the sample of synaptically connected pairs of spiny neurons in layer 4 (n = 131), ∼80% were identified as spiny stellate neurons and the remainder as star pyramidal neurons. However, often no clear distinction between the two cell types was possible because of the variability in the morphology and length of the apical dendrite. Representative examples of pairs of coupled spiny stellate (nine cell pairs) and star pyramidal neurons (two cell pairs) were selected for further analysis.
Spiny stellate cells
Spiny stellate cell dendrites in the barrel cortex have a characteristic asymmetric orientation (Figs. 2B,3A,4, 5), in contrast to spiny stellate cells in layer 4 of the visual cortex that generally display a multipolar, almost radially symmetric dendritic field (LeVay, 1973; Lund, 1984; Martin and Whitteridge, 1984; 1988; but see Katz et al., 1989; Kossel et al., 1995). Three to six thick primary dendrites emerged from the spherical to ovoid somata that gave rise to several secondary, tertiary, and higher-order dendrites. These dendrites formed an asymmetric dendritic field of various size (Table 1) that was confined to a single barrel and always oriented toward its center (Figs.2B, 3A, 4). Higher-order dendrites were densely covered with spines (Fig. 5). Spiny stellate cells that were synaptically coupled to each other as described here resembled those designated as class I spiny neurons in the barrel cortex by Woolsey and coworkers (Pasternak and Woolsey, 1975; Simons and Woolsey, 1984).
The axonal collaterals of spiny stellate cells project throughout all cortical laminae from layer 1 to the white matter (Figs. 3A,4) and remain largely confined to a single cortical column. The main axon emerges from the soma and descends toward the white matter, giving rise to numerous collaterals. Most of these collaterals branch off in layer 4 and ascend toward layer 2/3. In layers 5 and 6, a few long horizontal collaterals (length 500–800 μm) were observed that may project to adjacent cortical columns. The densest axonal projection was found in layers 4 and 2/3 where the axons show a high degree of collateralization. In these layers most of the axonal collaterals were confined to a single cortical column (Fig. 4). Their orientation is predominantly vertical in layers 2/3 and 4, whereas in layers 5 and 6 they follow a slightly descending horizontal course (Figs.3A, 4).
Putative synaptic contacts (two to five) (Feldmeyer et al., 1999b) were distributed over the entire dendritic tree but preferentially located on tertiary dendrites and relatively close to the soma (Fig. 5C). In addition, potential autaptic contacts were identified that displayed a similar dendritic distribution as the synapses.
To estimate the number of postsynaptic target neurons contacted by a single spiny stellate cell, the total number of synaptic boutons was counted separately for each cortical layer (Table2). More than 75% of all synaptic boutons were found in layers 4 and 2/3, with the highest density in layer 2/3; the remaining 25% of synaptic boutons were found in layers 5 and 6 (Table 2). This result suggests that the main target cells of spiny stellate cell axons are spiny neurons in layer 4 and pyramidal neurons in 2/3, implying that the flow of excitation is preferentially directed from layer 4 to layer 2/3. This view is further substantiated by the fact that the number of synaptic boutons per 100 μm axonal segment was significantly higher (p > 0.01) in layers 2/3 and 4 than in the other layers (Table3). Although we cannot exclude the possibility that boutons may also synapse on apical oblique dendrites of infragranular pyramidal neurons, the preferential termination of spiny stellate boutons appears to be on neurons in these layers.
Star pyramidal neurons
The second class of synaptically coupled excitatory neurons resembled those designated as star pyramidal cells (Lund, 1984; for review, see Lund, 1988). These neurons constitute a smaller fraction (∼20%) of the spiny neurons in layer 4 of the barrel cortex. Somata and dendritic domains of star pyramidal neurons were also exclusively located within layer 4, with the exception of the prominent apical dendrite. Its distal part often ascends to layer 2/3, but without forming a terminal tuft (Figs. 3B,6). In contrast to spiny stellate cells, star pyramidal cells never showed an asymmetry of the dendritic arbor (Figs. 3B, 6). Three to seven primary basal dendrites emerge from the spherical to ovoid soma that give rise to secondary, tertiary, and higher-order basal dendrites of various lengths. Most of the dendrites were restricted to a single barrel. The thick apical dendrite emerges from the upper pole of the soma and ascends through layer 4, giving rise to several oblique apical dendrites (Figs.3B, 6). The number and distribution of synaptic and autaptic contacts were similar to those of spiny stellate cells (see alsoFeldmeyer et al., 1999b, their Table 2).
The axons of star pyramidal cells projected also into all cortical layers (1–6) but spared the white matter (Figs. 3B, 6). As shown for spiny stellate cells, axonal collaterals were largely confined to a single cortical column. The main axon emerges either directly from the soma or from one of the primary basal dendrites and descends toward the white matter. In some neurons the main axon was seen to loop back toward layer 4 after reaching layer 6. The main axon gives rise to numerous collaterals ascending vertically toward layer 1. Only a few but long collaterals (up to 700 μm) were observed to descend to layers 5 and 6 (Figs. 3B, 6). Again, the most dense axonal projection was established in layers 4 and 2/3, but the density of collaterals and the degree in branching of the axonal collaterals were lower when compared with the axonal arborization of spiny stellate cells (compare Figs. 4 and 6). In layer 4, axonal collaterals are largely confined to a single barrel, whereas in upper layer 2/3 they fan out so that a few appear to project to adjacent cortical columns (Figs. 3B, 6). In upper layer 2/3 axonal collaterals were often organized in clusters, as described for pyramidal cells of cortical laminae 2/3 and 5 (Fig. 3B) (see also Gilbert and Wiesel, 1979). The total number of synaptic boutons on the axons of star pyramidal cells was significantly lower than that of spiny stellate cells (Table 2). This may be related to the lower number of axonal collaterals, because the number of boutons per 100 μm axonal segment was similar to that of spiny stellate cells (p > 0.01) (Table 3). Again, most of the synaptic boutons (∼70%) were found in layers 4 and 2/3, with the highest density in layer 2/3 (Table 2). The number of synaptic boutons per 100 μm axonal segment was also significantly higher (p > 0.01) in layers 2/3 than in layers 4 and 5 (Table 3). As observed for spiny stellate cells, star pyramidal neurons establish synaptic contacts predominantly with neurons in superficial layers 4 and 2/3 of the barrel cortex or superficial dendritic segments of infragranular pyramidal neurons traversing through these layers. This notion is supported by paired recordings between spiny layer 4 neurons and layer 2/3 pyramidal cells of the barrel cortex (Feldmeyer et al., 1999a).
Postsynaptic target structures of excitatory spiny neurons in layer 4 of the barrel cortex
The number of axonal collaterals as well as the density of synaptic boutons was highest in layers 4 and 2/3, suggesting that the main stream of excitation via spiny layer 4 neurons is directed to these layers. Synaptic contacts established by the axons of biocytin-labeled spiny neurons (n = 3) in layer 4 of the barrel cortex with postsynaptic target structures in layers 4 and 2/3 were examined in serial ultrathin sections. Of the total number of boutons investigated (n = 200; 75 in layer 4 and 125 in layer 2/3), the vast majority of the target structures in layers 4 and 2/3 were excitatory spiny neurons. This could explain the high probability in electrophysiological experiments of finding connected pairs of excitatory spiny neurons in layer 4 or between layers 4 and 2/3 (Feldmeyer et al., 1999a,b). In layer 4, most of the synaptic contacts (n = 55) were found on small caliber dendritic shafts (Fig. 7C,D) and a smaller fraction (n = 20) on dendritic spines (Fig. 7A) of other spiny neurons. In layer 2/3, synaptic contacts were formed with either small caliber dendritic shafts (n = 57) (Fig. 7F) or spines (n = 63) (Fig. 7E,G) of putative basal dendrites of layer 2/3 pyramidal neurons (n = 120) and on a smaller fraction with thick caliber apical dendrites (n = 5) of either layer 2/3 or layer 5 pyramidal neurons (Fig. 7H).
In addition, on every third grid, GABA postembedding immunogold labeling was performed to further identify GABAergic target structures of biocytin-labeled excitatory spiny cell axons. In the sample investigated (n = 60 sections), no biocytin-labeled boutons were found that synapsed on GABAergic profiles. However, in the same sample, GABAergic structures such as synapses, dendritic profiles, and somata that were not contacted by biocytin-labeled boutons could be easily identified (data not shown). Again, this finding suggests that the main target structures of excitatory spiny neurons are other excitatory spiny neurons in layer 4 and pyramidal neurons in layer 2/3.
DISCUSSION
The dendritic geometry, the axonal projections, and the postsynaptic target structures of excitatory spiny neurons in layer 4 of the barrel cortex provide the morphological basis for their functional role in the microcircuitry of a cortical column. We have sharpened the morphological picture of the excitatory microcircuits by using dual recording from synaptically connected pairs and subsequent characterization of the morphology of the spiny layer 4 neurons.
The results show that the dendritic arbor of synaptically coupled spiny layer 4 neurons is largely confined to a single barrel in layer 4 and that both synaptic and autaptic contacts were exclusively found within a barrel in layer 4, whereas their axon collaterals project throughout all cortical layers. The axonal collaterals were also largely confined to a single cortical column in the granular and supragranular layers. However, a few horizontal collaterals in layers 2/3, 5, and 6 project to adjacent cortical columns. The total number of synaptic boutons and their density per unit length of axon were highest in layers 2/3 and 4. These morphological findings suggest that the main target neurons of a spiny neuron in layer 4 are other excitatory spiny neurons in layer 4 of the same barrel and pyramidal neurons in layer 2/3 of the same cortical column (Feldmeyer et al., 1999a,b), and probably to a lesser extent pyramidal neurons in infragranular layers 5 and 6.
Axonal projection pattern and dendritic morphology of spiny layer 4 neurons
The axonal projection of spiny layer 4 neurons in the barrel cortex is highly organized with respect to the structure of a cortical column. In a quantitative Golgi study, Harris and Woolsey (1983) have shown that the main axonal trunk of class I neurons (corresponding to spiny layer 4 neurons) is directed toward the white matter, with recurrent collaterals projecting back into the barrels. Axonal projections to infragranular and supragranular layers were not reported, which may be attributable in part to the different plane of sectioning and incomplete staining of axonal collaterals by the Golgi method. Whole-cell recording in combination with intracellular biocytin labeling in the oblique coronal slice (Agmon and Connors, 1991) made it possible to describe the axonal projections of spiny layer 4 neurons in more detail.
The axonal projections of spiny layer 4 neurons in the visual cortex are well documented, in contrast to the barrel cortex (Martin and Whitteridge, 1984; Lund, 1988; Burkhalter, 1989; Ahmed et al., 1994). Spiny stellate and star pyramidal cells show a multitude of axonal projection patterns. Axons can either be more locally organized or display a patchy and extensive (2.5 mm lateral spread) tangential projection (Martin and Whitteridge, 1984, their Figures 8–10). This variability in projection patterns in layer 4 could be explained by the different information processing pathways for somatic/visceral and visual information as well as by different organization at the level of cortical layer 4 (barrels vs ocular dominance columns).
The dendritic arborization pattern of spiny neurons in layer 4 has been studied in detail previously (Pasternak and Woolsey, 1975; Woolsey et al., 1975; Steffen, 1976; Steffen and van der Loos, 1980; Harris and Woolsey, 1981; Simons and Woolsey, 1984). Asymmetry of the dendritic arborization has been noted for some but not all spiny layer 4 neurons (class I neuron). In this study, nearly all spiny stellate cells (∼95%) that were investigated showed a clear asymmetry, whereas star pyramidal neurons with a characteristic main apical trunk display a radially symmetric distribution of their basal dendrites. This classification was possible because the oblique coronal plane of sectioning allowed discrimination of spiny stellate and star pyramidal neurons in contrast to the tangential plane used in Golgi studies (Pasternak and Woolsey, 1975; Woolsey et al., 1975; Steffen, 1976;Simons and Woolsey, 1984). Because the axonal and the dendritic field span of a spiny stellate cell show a strong overlap and cover one-third to two-thirds of a barrel (∼200–400 μm in diameter), the strong asymmetry of the dendritic field could result in segregation of the inputs within an individual barrel. This appears to be unlikely for star pyramidal cells with a more radially symmetric dendritic field. In addition, these neurons may receive additional synaptic input via their apical dendrites.
Flow of excitation in the barrel cortex
Granular layer
The target structures of thalamic afferents arising from the ventroposterior medial nucleus are excitatory spiny neurons and different GABAergic interneurons in layer 4 (White et al., 1984;Benshalom and White, 1986). Apart from thalamic input, these neurons receive excitation from intracortical sources, namely other spiny layer 4 neurons and layer 6 pyramidal neurons (Benshalom and White, 1986). However, the contribution of thalamocortical versus intracortical projections to the excitatory drive of spiny layer 4 neurons is still a matter of debate. It has been demonstrated that thalamocortical afferents to spiny layer 4 neurons in the barrel cortex are characterized by a high reliability, whereas intracortical connections are supposedly of low reliability (Gil et al., 1999). However, synaptic transmission between individual spiny layer 4 neurons has a low failure rate, a low coefficient of variation, and a high connectivity (Feldmeyer et al., 1999b). This suggests that intracortical inputs serve to enhance even weak thalamic activity; the main excitatory drive thus appears to be generated intracortically (Douglas et al., 1995;Stratford et al., 1996; Feldmeyer et al., 1999b). Evidence supporting this hypothesis comes from Ahmed et al. (1994) who reported a more than fourfold preponderance of intracortical over thalamocortical inputs to spiny stellate neurons of cat visual cortex. Furthermore, Stratford et al. (1996) and Tarczy-Hornoch et al. (1999) found that both thalamocortical and intracortical (spiny stellate–spiny stellate connections) have a high reliability similar to those found in the somatosensory cortex.
Supragranular layers
Spiny layer 4 neurons subsequently relay excitation to layer 2/3 but because of the largely columnar organization of the axons of these neurons it remains restricted to neurons within the same cortical column (Feldmeyer et al., 1999a,b). This finding is further supported by optical recordings of voltage-sensitive dyes, which have shown that excitatory activity evoked by stimulation of thalamocortical afferents is largely restricted to a single barrel whereas in layer 2/3 it spreads across cortical columns (Laaris et al., 2000). It may be speculated that in layer 2/3 excitation arriving from layer 4 is distributed by pyramidal cell axons throughout the primary somatosensory cortex in vertical and horizontal directions (for review, see DeFelipe and Farinas, 1992). In supragranular layers, the spread of excitation may be no longer confined to a cortical column but mostly lateral to adjacent or even more distant cortical columns (Fig.8). Furthermore, excitatory activity is probably not restricted to one hemisphere but also relayed by the commissural axons of layer 2/3 pyramidal neurons via the corpus callosum to the other hemisphere (DeFelipe and Farinas, 1992). This may help to correlate and balance sensory input from the ipsilateral and the contralateral whisker pad. Obviously this spread of excitation depends mostly on the functional properties of spiny stellate and pyramidal cells that will filter excitation, depending on the frequency-dependent transmission properties (i.e., short-term plasticity) and spatial and temporal coincidence of synaptic activity in these neurons (Egger et al., 1999). This may represent the initial step in the cortical integration of afferent sensory signals from several whiskers. This proposal is supported by in vivo2-deoxyglucose mapping and imaging studies showing that the tangential spread of excitation occurs indeed at the level of layer 2/3 (McCasland and Woolsey, 1988; Kleinfeld and Delaney, 1996; Woolsey et al., 1996). Finally, layer 2/3 pyramidal cells can excite layer 5 pyramidal cells, the principal output neurons of the neocortex (Thomson and Bannister, 1998; Reyes and Sakmann, 1999).
Infragranular layers
In analogy to the visual cortex, spiny layer 4 neurons may also establish synaptic contacts with layer 6 pyramidal neurons and in turn may receive synapses from these neurons (Gilbert and Wiesel, 1979;Martin and Whitteridge, 1984; McGuire et al., 1984; Benshalom and White, 1986; Ahmed et al., 1994; Stratford et al., 1996; Tarczy-Hornoch et al., 1999). The axonal projection of spiny layer 4 neurons toward layer 6 makes it likely that such a feed-forward loop exists also in the somatosensory cortex and may also serve to control the flow of excitation.
Inhibitory neurons
The flow of excitation within a cortical column is controlled by a very heterogeneous population of GABAergic interneurons in each layer (Somogyi et al., 1998; Gupta et al., 2000). Based on the location of GABAergic synapses with excitatory principal neurons, interneurons have different functions, e.g., feedback–feedforward inhibition and suppression of dendritic Ca2+ spikes (Miles et al., 1996; Larkum et al., 1999). Several classes of GABAergic interneurons in the neocortex have been identified to date (Jones, 1993; Kawaguchi and Kubota, 1993, 1996, 1997; Deuchars and Thomson, 1995; Kawaguchi, 1995; Thomson et al., 1996; Tamás et al., 1997,1998; Reyes et al., 1998; Gupta et al., 2000), and electrophysiological recordings have demonstrated the existence of synaptic contacts between spiny layer 4 neurons and layer 4 interneurons (V. Egger, D. Feldmeyer, and B. Sakmann, unpublished results). However, their specific function in the columnar microcircuitry is still unclear. Recent evidence indicates that certain types of GABAergic interneurons are coupled via gap junctions (Galarreta and Hestrin, 1999; Gibson et al., 1999). This may support concerted activity of these neurons; however, it is still unknown which effects this may have on the flow of excitation in a cortical column.
Footnotes
This work was supported by the Deutsche Forschungsgemeinschaft (SFB 505/C6) and the Max-Planck-Society. We thank Dr. Imre Vida and Arnd Roth for critically reading an earlier version of this manuscript. We are also grateful to B. Joch, S. Nestel, M. Winter, and I. Dehof for excellent technical assistance.
Correspondence should be addressed to Dr. Joachim Lübke, Anatomisches Institut der Albert-Ludwigs-Universität Freiburg, Albertstraße 17, D-79104 Freiburg, Germany. E-mail:luebkejo{at}uni-freiburg.de.